Global ETD Search

41	Povrchová topografie a mechanické vlastnosti tenkých vrstev na bázi tetravinylsilanu / Surface topography and mechanical properties of thin films on tetravinylsilane basis Plichta, Tomáš January 2016 (has links) Proposed diploma thesis is focused on preparation and characterization of the plasma polymer thin films based on tetravinylsilane monomer (TVS). Plasma enhanced chemical vapour deposition (PECVD) method involving pulse and continual plasma discharge modes were used for thin film deposition on silicon wafer pieces. Reactive plasma composition was containing pure TVS or mixtures of TVS and argon or oxygen gas. Atomic force microscopy was used for surface topography and roughness characterization. Cyclic nanoindentation was involved to measurements to determine the Young’s modulus and hardness of prepared films and scratch test was performed to evaluate the degree of adhesion. Special attention was drawn to the characterization of films with a Young’s modulus below 10 GPa. Tip geometry of indenter influence on scratch test was also commented. Surface and mechanical properties of thin films in relation to the deposition conditions were correlated to the obtained results and final analysis of deposition conditions influence is proposed.
42	Epitaxy and characterization of SiGeC layers grown by reduced pressure chemical vapor deposition Hållstedt, Julius January 2004 (has links) Heteroepitaxial SiGeC layers have attracted immenseattention as a material for high frequency devices duringrecent years. The unique properties of integrating carbon inSiGe are the additional freedom for strain and bandgapengineering as well as allowing more aggressive device designdue to the potential for increased thermal budget duringprocessing. This work presents different issues on epitaxialgrowth, defect density, dopant incorporation and electricalproperties of SiGeC epitaxial layers, intended for variousdevice applications. Non-selective and selective epitaxial growth of Si1-x-yGexCy(0≤x≤30, ≤y≤0.02) layershave been optimized by using high-resolution x-ray reciprocallattice mapping. The incorporation of carbon into the SiGematrix was shown to be strongly sensitive to the growthparameters. As a consequence, a much smaller epitaxial processwindow compared to SiGe epitaxy was obtained. Differentsolutions to decrease the substrate pattern dependency (loadingeffect) of SiGeC growth have also been proposed. The key pointin these methods is based on reduction of surface migration ofthe adsorbed species on the oxide. In non-selective epitaxy,this was achieved by introducing a thin silicon polycrystallineseed layer on the oxide. The thickness of this seed layer had acrucial role on both the global and local loading effect, andon the epitaxial quality. Meanwhile, in selective epitaxy,polycrystalline stripes introduced around the oxide openingsact as migration barriers and reduce the loading effecteffectively. Chemical mechanical polishing (CMP) was performedto remove the polycrystalline stripes on the oxide. Incorporation and electrical properties of boron-doped Si1-x-yGexCylayers (x=0.23 and 0.28 with y=0 and 0.005) with aboron concentration in the range of 3x1018-1x1021atoms/cm3 have also been investigated. In SiGeClayers, the active boron concentration was obtained from thestrain compensation. It was also found that the boron atomshave a tendency to locate at substitutional sites morepreferentially compared to carbon. These findings led to anestimation of the Hall scattering factor of the SiGeC layers,which showed good agreement with theoretical calculations. Keywords:Silicon germanium carbon (SiGeC), Epitaxy,Chemical vapor deposition (CVD), Loading effect, Highresolution x-ray diffraction (HRXRD), Hall measurements, Atomicforce microscopy (AFM). Silicon germanium carbon (SiGeC) Epitaxy Chemical vapor deposition (CVD) Loading effect Hall measurements Atomic force microscopy (AFM).
43	Fundamental Analysis of the Interaction of Low Pressure Plasmas with Polymer Surfaces Bach, Markus 25 November 2003 (has links) The treatment of polymer surfaces by low pressure plasmas is of technological interest in a variety of applications for modification and functionalisation. Until now the interactions of the individual plasma species (especially electrons) with polymeric material have not been subject of a microscopic study.In an anticipated chapter the inner plasma parameters were characterised by Langmuir probe measurements, leading to a precise knowledge about the density and energy distributions of plasma electrons and ions. The values for electrons were later used for an exclusive treatment with this species. The main part of this thesis describes and interprets the chemical composition after UV, plasma and electron treatment by x-ray photoelectron spectroscopy (XPS), structural changes by atomic force microscopy (AFM) and their combination to distinguish the fundamental interactions with polyethylene and polypropylene surfaces. It was found that all treatments show specific modification behaviour according to the chemical composition, topography and modification depth. For an argon microwave discharge, the plasma effects can also be obtained by a combination of UV and electron treatment. Fundamental radical reactions have been traced indirectly by chemical derivatisation as well as their passivation reactions through cross-linkage and the creation of double bonds. X-ray photoelectron spectroscopy (XPS) atomic force microscopy (AFM) Langmuir probe measurements plasma surface treatment polymers 29 - Physik, Astronomie ddc:530
44	Controlled orientation and periodicity of surface rippling on compliant and brittle amorphous materials induced by scanning probe lithography Hennig, Jana 21 March 2023 (has links) This thesis reports on the controlled formation of surface rippling structures induced by tip scanning processes on compliant and brittle materials. Periodic surface structures were generated on polymeric and vitreous materials and with different length scales. Two aspects were focused on: the controlling of orientation and periodicity of the resulting structures via proper tuning the scan conditions and the physical mechanisms ruling the early stages of plowing wear causing the rippling effect. Specifically the influence of the scanned area geometric shape on the orientation of the rippling structure was investigated on a polystyrene surface. Nanoripples were induced by scanning the surface with a silicon tip using atomic force microscopy and dedicated scripts. Inside a structured area two ripple orientations can be observed: near boundaries the ripple orientation is determined by boundary orientation and regions away from the boundaries the ripples are aligned in a steady orientation. This steady orientation can be tuned by the distance between the scan lines. In the boundary regions the orientation of the ripples is different from steady orientation. The orientation of the boundaries clearly affected the orientation of the ripples and the tendency of the ripples to align in a steady angle defined by the scan parameters could be significantly modified. Geometric shapes like squares, circles, stars, pentagons and hearts allowed to distinguish the influence of curved and straight boundaries. Straight boundaries with different orientations allowed a detailed analysis of the influence of the angle on the rippling process. Straight boundaries inclined in the direction of the steady state angle of ripple orientation previously defined generate a uniform ripple pattern covering the entire scan area. The aspect of wear originating from the rippled surface was also investigated on similar polystyrene surfaces. As a result of repetitive scan passes spherical particles with diameters up to 250 nm were nucleated and detached from the surface. The particles originate from the crests of the ripples formed in the first scan pass. As proven by the lateral force signal the detachment occurs smoothly without a static friction peak suggesting a crazing mechanism induced by the scanning tip. Once detached from the surface the particles are displaced and piled up along the edges of scanned area. The formation of periodic surface structures was also investigated on a brittle silica glass. By a combination of scratch tests performed with a diamond microtip mounted in a nanoindenter and imaging with atomic force microscopy the existence of a periodic herringbone pattern inside scratch grooves on silica glass was proven. The rippled pattern was induced in the scratch process when the indenter was pulled laterally along the surface resulting in a microscopic scratch groove. The load was varied up to 30 nN and the scan velocity up to 500 µm/s. The resulting periodicity of the structures was found to increase linearly with increasing scratch velocity. The repetition distance was in the range of sub-µm and the corrugation in the range of a few hundred nm, which was well below indentation depth. In both cases, the surface rippling on a polymeric surfaces and the formation of a periodic pattern inside microscratches on a glass surface, the results were found to be consistent with minimalistic theoretical models for stick-slip.:Contents i Abstract iii Zusammenfassung v 1. Introduction 1 1.1. Periodic surface structures – relevance and formation 1 1.2. Surface rippling created by scanning probe lithography 2 1.3. Wear and nanoparticle release 4 1.4. Aim and outline 4 2. Experimental methods and fundamental concepts 6 2.1. Nanolithography 6 2.2. Atomic force microscopy 7 2.3. Nanoindentation and -scratching 10 2.4. Wear 11 2.5. Stick-slip motion 12 2.6. Spin coating 14 3. Surface rippling on polystyrene 15 3.1. Background and motivation 15 3.2. Methods 20 3.2.1. Sample preparation 20 3.2.2. Scanning probe lithography process 20 3.2.3. Imaging of structures and nanoparticles 21 3.3. Effect of boundaries on the orientation of surface rippling 22 3.4. Particle release as a result of surface rippling 31 4. Periodic structures inside scratches on silica glass 37 4.1. Background and motivation 37 4.2. Methods 38 4.2.1. Sample preparation 39 4.2.2. Scratch tests 39 4.2.3. AFM imaging and analysis 39 4.3. Surface rippling induces by scraping with a sharp indenter 40 5. Conclusion and outlook 49 A. Appendix surface rippling on polymers I B. Appendix surface rippling on glass IV Acknowledgements VII References IX info:eu-repo/classification/ddc/620 ddc:620
45	Single Cell Biomechanical Phenotyping using Microfluidics and Nanotechnology Babahosseini, Hesam 20 January 2016 (has links) Cancer progression is accompanied with alterations in the cell biomechanical phenotype, including changes in cell structure, morphology, and responses to microenvironmental stress. These alterations result in an increased deformability of transformed cells and reduced resistance to mechanical stimuli, enabling motility and invasion. Therefore, single cell biomechanical properties could be served as a powerful label-free biomarker for effective characterization and early detection of single cancer cells. Advances and innovations in microsystems and nanotechnology have facilitated interrogation of the biomechanical properties of single cells to predict their tumorigenicity, metastatic potential, and health state. This dissertation utilized Atomic Force Microscopy (AFM) for the cell biomechanical phenotyping for cancer diagnosis and early detection, efficacy screening of potential chemotherapeutic agents, and also cancer stem-like/tumor initiating cells (CSC/TICs) characterization as the critical topics received intensive attention in the search for effective cancer treatment. Our findings demonstrated the capability of exogenous sphingosine to revert the aberrant biomechanics of aggressive cells and showed a unique, mechanically homogeneous, and extremely soft characteristic of CSC/TICs, suitable for their targeted isolation. To make full use of cell biomechanical cues, this dissertation also considered the application of nonlinear viscoelastic models such as Fractional Zener and Generalized Maxwell models for the naturally complex, heterogeneous, and nonlinear structure of living cells. The emerging need for a high-throughput clinically relevant alternative for evaluating biomechanics of individual cells led us to the development of a microfluidic system. Therefore, a high-throughput, label-free, automated microfluidic chip was developed to investigate the biophysical (biomechanical-bioelectrical) markers of normal and malignant cells. Most importantly, this dissertation also explored the biomechanical response of cells upon a dynamic loading instead of a typical transient stress. Notably, metastatic and non-metastatic cells subjected to a pulsed stress regimen exerted by AFM exhibited distinct biomechanical responses. While non-metastatic cells showed an increase in their resistance against deformation and resulted in strain-stiffening behavior, metastatic cells responded by losing their resistance and yielded slight strain-softening. Ultimately, a second generation microfluidic chip called an iterative mechanical characteristics (iMECH) analyzer consisting of a series of constriction channels for simulating the dynamic stress paradigm was developed which could reproduce the same stiffening/softening trends of non-metastatic and metastatic cells, respectively. Therefore, for the first time, the use of dynamic loading paradigm to evaluate cell biomechanical responses was used as a new signature to predict malignancy or normalcy at a single-cell level with a high (~95%) confidence level. / Ph. D. MicroElectroMechanical Systems (MEMS) Biomechanics Microfluidics Atomic Force Microscopy (AFM) Drug Screening Tumor Initiating Cells Fractional Zener Model Generalized Maxwell Model Single Cell Analysis Pulsed Stress iMECH Cancer
46	Identification of Cell Biomechanical Signatures Using Three Dimensional Isotropic Microstructures Nikkhah, Mehdi 28 December 2010 (has links) Micro and nanofabrication technologies have been used extensively in many biomedical and biological applications. Integration of MEMS technology and biology (BioMEMS) enables precise control of the cellular microenvironments and offers high throughput systems. The focus of this research was to develop three dimensional (3-D) isotropic microstructures for comprehensive analysis on cell-substrate interactions. The aim was to investigate whether the normal and cancerous cells differentially respond to their underlying substrate and whether the differential response of the cells leads to a novel label-free technique to distinguish between normal and cancerous cells. Three different generations of 3-D isotropic microstructures comprised of curved surfaces were developed using a single-mask, single-etch step process. Our experimental model included HS68 normal human fibroblasts, MCF10A normal human breast epithelial cells and MDA-MB-231 metastatic human breast cancer cells. Primary findings on the first generation of silicon substrates demonstrated a distinct adhesion and growth behavior in HS68 and MDA-MB-231 cells. MDA-MB-231 cells deformed while the fibroblasts stretched and elongated their cytoskeleton on the curved surfaces. Unlike fibroblasts, MDA-MB-231 cells mainly trapped and localized inside the deep microchambers. Detailed investigations on cytoskeletal organization, adhesion pattern and morphology of the cells on the second generation of the silicon substrates demonstrated that cytoskeletal prestress and microtubules organization in HS68 cells, cell-cell junction and cell-substrate adhesion strength in MCF10A cells, and deformability of MDA-MB-231 cells (obtained by using AFM technique) affect their behavior inside the etched cavities. Treatment of MDA-MB-231 cells with experimental breast cancer drug, SAHA, on the second generation of substrates, significantly altered the cells morphology, cytoarchitecture and adhesion pattern inside the 3-D microstructures. Third generation of silicon substrates was developed for comprehensive analysis on behavior of MDA-MB-231 and MCF10A cells in a co-culture system in response to SAHA drug. Formation of colonies of both cell types was evident inside the cavities within a few hours after seeding the cells on the chips. SAHA selectively altered the morphology and cytoarchitecture in MDA-MB-231 cells. Most importantly, the majority of MDA-MB-231 cells stretched inside the etched cavities, while the adhesion pattern of MCF10A cells remained unaltered. In the last part of this dissertation, using AFM analysis, we showed that the growth medium composition has a pronounced effect on cell elasticity. Our findings demonstrated that the proposed isotropic silicon microstructures have potential applications in development of biosensor platforms for cell segregation as well as conducting fundamental biological studies. / Ph. D. HS68 MCF10A Silicon Atomic Force Microscopy (AFM) MDA-MB-231 Breast Cancer Suberoylanilide Hydroxamic Acid (SAHA) Isotropic Three Dimensional (3-D) MicroElectroMechanical Systems (MEMS)
47	Nanolithographie par sonde locale catalytique : une approche bottom-up pour la nanostructuration de surfaces organominérales / Catalytic scanning probe lithography : a bottom-up approach allowing the nanostructuration of organomineral surfaces Botton, Julien 17 December 2015 (has links) Face à la quête constante de miniaturisation, les nanosciences ont connu un essor fulgurant lors de la dernière décennie. Au sein de ces dernières, les procédés lithographiques – clé de voûte de l’industrie des semi-conducteurs – permettent désormais d’accéder à des nanomatériaux fonctionnels. Malgré les récents développements technologiques, l’obtention de nanostructures possédant une résolution inférieure à 100 nm reste un défi majeur pour la communauté scientifique.Devant l’intérêt grandissant de développer des méthodes alternatives en nanolithographie, notre groupe s’est tourné vers une approche chimique, nommée nanolithographie par sonde locale catalytique (cSPL). Combinant la robustesse de la catalyse organométallique et la flexibilité offerte par la microscopie à sonde locale, notre stratégie permet la nanostructuration de surfaces organominérales par la création de liaisons covalentes dans des conditions douces. Cette approche innovante constitue le premier exemple d’immobilisation d’un catalyseur homogène à la surface d’une pointe d’un microscope à force atomique (AFM), dans l’optique de contrôler spatialement une réactivité chimique, l’époxydation localisée d’alcènes terminaux. Ces fonctions époxydes ont été employées comme points d’ancrage dans la nanostructuration à façon de surfaces de silicium avec une large variété de nucléophiles. De plus, l’optimisation des paramètres physico-chimique influant sur la réaction, a permis d’atteindre des résolutions latérales de l’ordre de 40 nm et laisse entrevoir de nombreuses perspectives dans la nanostructuration tridimensionnelle de matériaux organiques. / In regard to the constant quest for miniaturization, the field of nanosciences has known a tremendous expansion over the last decade. More precisely, lithographic technologies - key processes for the semi-conductor industry – allow to access to functional nanomaterials. Despite recent technological developments, the synthesis of nanostructures with a sub-100 nm resolution remains a major challenge for the scientific community.Due to the growing interest in the design of new nanolithographic methods, our group has focused its efforts on the development of a chemical approach, named catalytic scanning probe lithography (cSPL). Unifying the robustness of organometallic catalysis and the flexibility offered by scanning probe microscopy, our strategy allows the nanostructuration of organomineral surfaces in a soft controlled manner by the formation of covalent bonds. This innovative approach represents the first example of the immobilization of an homogeneous catalyst on the edge of an atomic force microscope (AFM) tip, in order to spatially control a chemical reaction: the localized epoxidation reaction of terminal alkenes. Those epoxides were then used as anchoring sites, in the nanostructuration of silicon wafers with a broad range of nucleophiles. Moreover, the different physico-chemical parameters influencing the reaction were optimized, allowing us to reach lateral resolutions down to 40 nm and opening new perspectives in the field of 3D-nanostructuration of organic materials. Catalyse organométallique Époxydation localisée Microscopie à force atomique (AFM) Nanostructuration 3D Monocouche auto-Assemblée (SAM) Organometallic catalysis Localized epoxidation Atomic force microscopy (AFM) 3D nanostructuration Self-Assembled monolayers (SAM)
48	Light emitting organic nanofibers from para-phenylene and alpha-thiophene oligomers Kankate, Laxman 26 May 2008 (has links) Wir haben blau, grün und orange leuchtende organische Nanofäden oder Nanonadeln und Mikroringe aus para-Hexaphenyl (p-6P), alpha-Quaterthiophen (alpha-4T) und alpha-Sexithiophen (alpha-6T) mittels Organischer Molekularstrahlepitaxie (OMBE) auf Muskovit Glimmer hergestellt. Die Aggregate haben wir mit der Atomkraftmikroskopie, mit der Fluoreszenz-Mikroskopie und durch UV-vis Spektroskopie charakterisiert. Auf der Muskovit Oberfläche wachsen p-6P Fäden parallel zueinander auf und zeigen zwei verschiedene Orientierungsdomänen entlang [110] und [1-10]. Mit Hilfe einer systematischen statistischen Analyse diskutieren wir das Wachstum dieser p-6P Nadeln für verschiedene Wachstumsbedingungen. Zusätzlich zu den Fäden haben wir p-6P Cluster auf der Oberfläche beobachtet. Nadeln werden durch die Aggregation solcher Cluster gebildet. Ein Realraummodell der Morphologie der Nadeln sowie ein Modell für deren Wachstum werden vorgestellt. Indem wir Glimmer zunächst mit einer dünnen Goldschicht bedecken und die Wachstumsparameter variieren, erreichen wir eine weitgehende Kontrolle der Morphologie der Nadeln (Länge von 0,5 Mikrometer bis 1 mm, Höhe von 25 bis 300 nm und Breite von 100 bis 600 nm). Im Gegensatz zu p-6P orientieren Thiophene ihre Wachstumsrichtungen an allen hoch symmetrischen Richtungen von Glimmer. Es wird gezeigt, dass die Mechanismen für das Fadenwachstum von beiden Oligomere gleich sind, nämlich eine Kombination aus Epitaxie und einer Dipol-unterstützten Ausrichtung. Auch die Strukturen dieser Fäden sind ähnlich: die Moleküle liegen parallel angeordnet auf der Oberfläche, ihre Längsachsen orientieren sich schräg zur Längsachse der Fäden. Auf mit Wasser oder Methanol vorbehandeltem Glimmer wachsen diese beiden Oligomere als gebogene Fäden und Mikroringe auf. Diese Oberflächenvorbehandlungen sowie das Wachstum von p-6P auf Gold/Glimmer unterstützen auch den Wachstumsmechanismus auf der sauberen Glimmer-Oberfläche. / By using organic molecular beam epitaxy (OMBE) blue, green and orange light emitting organic nanofibers or nanoneedles and microrings from para-hexaphenyl (p-6P), alpha-quaterthiophene (alpha-4T) and alpha-sexithiophene (alpha-6T), respectively, on muscovite mica surfaces are generated. The aggregates are characterized by atomic force microscopy, fluorescence microscopy and UV-vis spectroscopy. On muscovite mica, p-6P fibers usually grow mutually parallel showing two domains of their orientations with an angle of 120 degree in between. The detail growth of nanofibers from p-6P by performing a systematic statistical analysis of fibers as a function of various growth conditions is discussed. Furthermore, the morphology exhibits p-6P clusters, which are found to be fibers´ building blocks. A real space model of the fiber and a model for their growth are also presented. By introducing a thin gold layer on mica prior to p-6P deposition together with varying growth parameters, the morphology of fibers is controlled in a wide range (length from 0.5 micrometer to 1 mm, height from 25 to 300 nm and width from 100 to 600 nm). In contrast to p-6P, thiophene fibers exhibit various orientations close to mica high symmetry directions. It is shown that the mechanism behind the fiber growth from all molecules on mica is the same, i.e. a combination of epitaxy and dipole assisted growth process. The fiber microscopic structures are similar, too: molecules take lying orientations and they hold themselves parallel pointing their long axes along an oblique direction off the long fiber axis. The growth of both types of oligomers on water or methanol treated mica surfaces leads to the formation of bent fibers and microrings. This surface pretreatment and the growth of p-6P on gold/mica support the fiber growth mechanism on plain mica. Nanofäden oder Nanonadeln Muskovit Glimmer para-Phenylene alpha-Thiophene statistische Analyse Molekül-Orientierung Atomkraftmikroskopie (AFM)) Nanofibers or nanoneedles muscovite mica para-phenylenes alpha-thiophenes statistical analysis molecular orientation atomic force microscopy (AFM) 530 Physik 29 Physik, Astronomie ddc:530
49	Quantifying adhesive interactions between cells and extracellular matrix by single-cell force spectroscopy Taubenberger, Anna Verena 08 October 2009 (has links) (PDF) Interactions of cells with their environment regulate important cellular functions and are required for the organization of cells into tissues and complex organisms. These interactions involve different types of adhesion receptors. Interactions with extracellular matrix (ECM) proteins are mainly mediated by the integrin family of adhesion molecules. Situations in which integrin-ECM interactions are deregulated cause diseases and play a crucial role in cancer cell invasion. Thus, the mechanisms underlying integrin-binding and regulation are of high interest, particularly at the molecular level. How can cell-ECM interactions be studied? While there are several methods to analyze cell adhesion, few provide quantitative data on adhesion forces. One group, single-cell force spectroscopy (SCFS), quantifies adhesion at the single-cell level and can therefore differentiate the adhesive properties of individual cells. One implementation of SCFS is based on atomic force microscopy (AFM); this technique has been employed in the presented work. Advantageously AFM-SCFS combines high temporal and spatial cell manipulation, the ability to measure a large range of adhesion forces and sufficiently high-force resolution to allow the study of single-molecule binding events in the context of a living cell. Since individual adhesion receptors can be analyzed within their physiological environment, AFM-SCFS is a powerful tool to study the mechanisms underlying integrin-regulation. The presented work is split into six chapters. Chapter one gives background information about cell-ECM interactions. In chapter two, different adhesion assays are compared and contrasted. The theoretical Bell-Evans model which is used to interpret integrin-mediated cell adhesion is discussed in chapter three. Thereafter, the three projects that form the core of the thesis are detailed in chapters four through six. In the first project (chapter 4), α2β1-integrin mediated cell adhesion to collagen type I, the most abundant structural protein in vertebrates, was quantified using CHO cells. Firstly, α2β1-collagen interactions were investigated at the single-molecule level. Dynamic force spectroscopy permitted calculation of bond specific parameters, such as the bond dissociation rate koff (1.3 ± 1.3 sec-1) and the barrier width xu (2.3 ± 0.3 Å). Next, α2β1-integrin mediated cell adhesion to collagen type I was monitored over contact times between 0 and 600 sec. Thereby the kinetics of α2β1-integrin mediated interactions was explored and insights into the underlying binding mechanisms were gained. In the second project (chapter five), effects of cryptic integrin binding sites within collagen type I exerted on pre-osteoblasts were investigated. Collagen type I matrices were thermally denatured which lead to exposure of cryptic RGD (Arg-Gly-Asp)-motifs. As a consequence pre-osteoblasts enhanced their adhesion to denatured collagen. Compared to native collagen type I, adhesion to denatured collagen was mediated by a different set of integrins, including αv- and α5β1-integrins. Cells grown on denatured collagen showed enhanced spreading and motility, which correlated with increased focal adhesion kinase phosphorylation levels. Moreover, osteogenic differentiation kinetics and differentiation potential were increased on denatured collagen. The findings of this project open new perspectives for optimization of tissue engineering substrates. In the third part (chapter six), the effect of the fusion protein BCR/ABL, a hallmark of chronic myeloid leukemia, on adhesion of myeloid progenitor cells was studied. Adhesion between BCR/ABL transformed progenitor cells to bone marrow derived stromal cells and to different ECM proteins was quantitatively compared to that of control cells. The tyrosine kinase activity of BCR/ABL enhanced cell adhesion, which was blocked by imatinib mesylate, a drug interfering with BCR/ABL activity. BCR/ABL-enhanced adhesion correlated with increased β1-integrin cell surface concentrations. Since adhesion of leukemic cells to the bone marrow compartment is critical for the development of drug resistance, the reported results may provide a basis for optimized target therapies. In the three described projects AFM-based SCFS was applied to investigate early steps of integrin-mediated adhesion at the molecular level. Taken together, the results demonstrate that AFM-SCFS is a versatile tool that permits monitoring of cell adhesion from single-molecule interactions to the formation of more complex adhesion sites at the force level. / Interaktionen zwischen Zellen und ihrer Umgebung sind maßgeblich an der Regulierung zellulärer Funktionen beteiligt und daher notwendig für die Organisation von Zellen in Geweben und komplexen Organismen. Zellinteraktionen mit der extrazellulären Matrix (EZM) werden hauptsächlich durch Integrine vermittelt. Situationen, in denen Integrin- EZM Interaktionen verändert sind, können Krankheiten verursachen und spielen zudem eine wichtige Rolle bei der Invasion von Krebszellen. Daher besteht ein großes Interesse darin, die molekularen Mechanismen, die Integrin-EZM Interaktionen regulieren, besser zu verstehen. Wie können Zell-EZM Interaktionen untersucht werden? Obwohl es mehrere Methoden gibt, mit denen Zelladhäsion untersucht werden kann, sind die wenigsten dazu geeignet, Zelladhäsionskräfte zu quantifizieren. Einzelzellspektroskopie erfasst die Adhäsionskräfte einzelner Zellen quantitativ und ermöglicht dadurch eine differenzierte Betrachtung der Adhäsion individueller Zellen. Eine Variante der Einzelzellspektroskopie basiert auf der Rasterkraftmikroskopie (AFM); diese Technik wurde in der vorliegenden Arbeit verwendet. Ein Vorteil von AFM- Einzelzellspektroskopie besteht darin, dass Zellen mit hoher zeitlicher und räumlicher Präzision manipuliert werden können. Zelladhäsionskräfte können zudem über einen großen Kraftbereich hinweg untersucht werden. Dabei ermöglicht es die hohe Kraftauflösung, einzelne Integrin-Ligandenbindungen in lebenden Zellen zu untersuchen. Die vorliegende Arbeit gliedert sich in sechs Kapitel. Kapitel eins gibt Hintergrundinformationen über Zell-EZM Wechselwirkungen. In Kapitel zwei werden verschiedene Adhäsionsassays einander gegenüber gestellt. Das theoretische Bell-Evans Modell, mit dessen Hilfe die gewonnenen Daten interpretiert wurden, wird in Kapitel drei diskutiert. Im Anschluss werden drei Projekte, welche das Herzstück dieser Doktorarbeit bilden, in Kapiteln vier bis sechs näher ausgeführt. Im ersten Projekt (Kapitel vier) wurde die Adhäsion von α2β1-Integrin exprimierenden CHO Zellen zu Kollagen I, dem häufigsten strukturellen Protein in Wirbeltieren, quantitativ untersucht. Zunächst wurden α2β1-Kollagen-Interaktionen auf Einzelmolekülebene analysiert. Mithilfe der dynamischen Kraftspektroskopie wurden für diese Bindung Dissoziationsrate koff (1.3 ± 1.3 sec-1) und Potentialbarrierenbreite xu (2.3 ± 0.3 Å) bestimmt. Daraufhin wurde die α2β1-vermittelte Adhäsion über einen Zeitraum von zehn Minuten untersucht. Dadurch konnten Einblicke in die Kinetik von α2β1-integrin vermittelter Zelladhäsion sowie in die zugrunde liegenden Regulationsmechanismen gewonnen werden. Im zweiten Projekt (Kapitel fünf) wurde die Rolle von kryptischen Integrin-Bindungsstellen in Kollagen I untersucht. Die zuvor verwendeten Kollagenoberflächen wurden thermisch denaturiert, wodurch versteckte RGD (Arg-Gly-Asp)-Sequenzen freigelegt wurden. Die partielle Denaturierung hatte- verglichen mit nativem Kollagen I- eine erhöhte Adhäsion von Präosteoblasten (MC3T3-E1) zur Folge, was auf das Binden zusätzlicher Integrine zurückgeführt wurde. Im Unterschied zu nativem Kollagen wurde die Zelladhäsion zu denaturiertem Kollagen I u.a. durch αv- and α5β1-Integrine vermittelt. Präosteoblasten zeigten verstärktes Zellspreiten sowie höhere Motilität auf denaturiertem Kollagen I; zudem wurde ein erhöhtes Differenzierungpotential der Präosteoblasten festgestellt. Die in diesem Projekt erhaltenen Einblicke bilden eine hilfreiche Basis für die Entwicklung optimierter Oberflächen für diverse Zell- und Gewebekulturanwendungen. Im dritten Projekt (Kapitel sechs) wurde der Einfluss des Fusionproteins BCR/ABL, charakteristisch für chronische myeloische Leukämie, auf die Adhäsion von myeloischen Vorläuferzellen untersucht. Dazu wurde die Adhäsion von BCR/ABL transformierten Vorläuferzellen (32D Zellen) bzw. Kontrollzellen zu Stromazellen (M2-10B4) sowie verschiedenen EZM Proteinen untersucht. BCR/ABL erhöhte die Zelladhäsion der myeloischen Vorläuferzellen signifikant. Dieser Effekt wurde durch die Zugabe von Imatinib, welches die Tyrosinkinaseaktivität von BCR/ABL inhibiert, aufgehoben. Die BCR/ABL-verstärkte Zelladhäsion korrelierte mit erhöhten β1-Integrin-konzentrationen. Da die Adhäsion von Leukämiezellen im Knockenmark bekanntermaßen kritisch für die Entwicklung von Resistenzen gegenüber verschiedenen Wirkstoffen ist, könnten die Ergebnisse dieser Studie eine Grundlage für die Entwicklung optimierter Target-Therapien sein. In den drei beschriebenen Projekten wurde AFM Einzelzellspektroskopie verwendet, um Integrin- vermittelte Adhäsion auf molekularer Ebene zu untersuchen. Die Ergebnisse zeigen, dass AFM-Einzelzellspektroskopie ein vielseitiges Werkzeug darstellt, das überaus geeignet dazu ist, Zelladhäsion- ausgehend von Einzelmolekülinteraktionen bis hin zur Entstehung komplexerer Adhäsionsstellen- auf der Kraftebene zu verfolgen. cell adhesion atomic force microscopy (AFM) single-cell force spectroscopy integrins extracellular matrix collagen type I Zelladhäsion Rasterkraftmikroskopie (AFM) Einzelzellkraftspektroskopie Integrine Extrazeluläre Matrix Kollagen I ddc:620 rvk:WE 2301
50	Interaction of the human N-Ras protein with lipid raft model membranes of varying degrees of complexity Vogel, Alexander, Nikolaus, Jörg, Weise, Katrin, Triola, Gemma, Waldmann, Herbert, Winter, Roland, Herrmann, Andreas, Huster, Daniel 07 December 2015 (has links) (PDF) Ternary lipid mixtures composed of cholesterol, saturated (frequently with sphingosine backbone), and unsaturated phospholipids show stable phase separation and are often used as model systems of lipid rafts. Yet, their ability to reproduce raft properties and function is still debated. We investigated the properties and functional aspects of three lipid raft model systems of varying degrees of biological relevance – PSM/POPC/Chol, DPPC/POPC/Chol, and DPPC/DOPC/Chol – using 2H solidstate nuclear magnetic resonance (NMR) spectroscopy, fluorescence microscopy, and atomic force microscopy. While some minor differences were observed, the general behavior and properties of all three model mixtures were similar to previously investigated influenza envelope lipid membranes, which closely mimic the lipid composition of biological membranes. For the investigation of the functional aspects, we employed the human N-Ras protein, which is posttranslationally modified by two lipid modifications that anchor the protein to the membrane. It was previously shown that N-Ras preferentially resides in liquid-disordered domains and exhibits a time-dependent accumulation in the domain boundaries of influenza envelope lipid membranes. For all three model mixtures, we observed the same membrane partitioning behavior for N-Ras. Therefore, we conclude that even relatively simple models of raft membranes are able to reproduce many of their specific properties and functions. Kernresonanz-Spektroskopie (NMR) Atomkraftmikroskopie (AFM) Membranprotein Ordnungsparameter atomic force microscopy (AFM) membrane protein order parameter ddc:570

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